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Phosphorylation of H2AX histone as indirect evidence for double-stranded DNA breaks related to the exchange of nuclear proteins and chromatin remodeling in Chara vulgaris spermiogenesis

机译:H2AX组蛋白的磷酸化作为双链DNA断裂的间接证据,与寻常型Chara精子发生过程中核蛋白的交换和染色质重塑有关

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摘要

Phosphorylation of H2AX histone results not only from DNA damage (caused by ionizing radiation, UV or chemical substances, e.g. hydroxyurea), but also regularly takes place during spermiogenesis, enabling correct chromatin remodeling. Immunocytochemical analysis using antibodies against H2AX histone phosphorylated at serine 139 indirectly revealed endogenous double-stranded DNA breaks in Chara vulgaris spermatids in mid-spermiogenesis (stages V, VI and VII), when protamine-type proteins appear in the nucleus. Fluorescent foci were not observed in early (stages I–IV) and late (VIII–X) spermiogenesis, after replacement of histones by protamine-type proteins was finished. A similar phenomenon exists in animals. Determination of the localization of fluorescent foci and the ultrastructure of nuclei led to the hypothesis that DNA breaks at stage V, when condensed chromatin adheres to the nuclear envelope. This is transformed into a net-like structure during stage VI, probably allowing chromosome repositioning to specific regions in the mature spermatozoid. However, at stages VI and VII, DNA breaks are necessary for transformation of the nucleosomal structure into a fibrillar and finally the extremely condensed status of sleeping genes at stage X.
机译:H2AX组蛋白的磷酸化不仅是由于DNA损伤(由电离辐射,紫外线或化学物质(例如羟基脲)引起)造成的,而且还经常在精子发生过程中发生,从而实现正确的染色质重塑。使用抗H2AX组蛋白在丝氨酸139处磷酸化的抗体进行的免疫细胞化学分析间接揭示了在精子形成中期(阶段V,VI和VII),当精蛋白类型的蛋白出现在核中时,寻常型Chara spermatids的内源双链DNA断裂。在完成鱼精蛋白类蛋白的组蛋白置换后,在早期(I–IV期)和晚期(VIII–X)精子发生过程中未观察到荧光灶。动物中也存在类似现象。荧光焦点的定位和细胞核的超微结构的确定导致了这样一个假说:当浓缩的染色质粘附在核膜上时,DNA在V期断裂。在第六阶段将其转变成网状结构,可能使染色体重新定位到成熟的精子中的特定区域。然而,在第VI和VII阶段,DNA断裂对于将核小体结构转化为原纤维以及最终在X阶段睡眠基因的高度浓缩状态是必需的。

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